首页> 外文期刊>Methods: A Companion to Methods in Enzymology >Confocal imaging of microglial cell dynamics in hippocampal slice cultures.
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Confocal imaging of microglial cell dynamics in hippocampal slice cultures.

机译:海马切片培养物中小胶质细胞动力学的共聚焦成像。

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Methods are described for imaging the cellular dynamics of microglia in live mammalian brain slice cultures. Brain slices prepared from developing rat hippocampus are cultured for up to 2 weeks by the roller tube or static filter culture technique, stained with one or more fluorescent dyes, and imaged by scanning laser confocal microscopy. One of several cell type-specific or nonspecific fluorescent dyes can be used independently or in combination to label cells in live brain tissues. The fluorescently conjugated plant isolectin GSA-IB4 is useful for identifying microglia and for following their structure, movement, and proliferation. Live and dead neurons and glia can be distinguished using membrane-permeant and -impermeant fluorescent nucleic acid dyes. Nonspecific fluorescent lipids such as DiIC18 can be used as a vital stain to label populations of endocytic and phagocytic cells. Using multichannel confocal imaging, tissue slices that are single-, double-, or triple-labeled can be imaged in the living state in two or three spatial dimensions as well as in time. This provides a means for investigating the cell-cell interaction and dynamic behavior of microglia and other cell types in live brain tissues cultured under various physiological conditions. Copyright 1999 Academic Press.
机译:描述了用于在活的哺乳动物脑切片培养物中对小胶质细胞动力学进行成像的方法。用滚管或静态滤器培养技术将由发育中的大鼠海马体制备的脑片培养最多2周,用一种或多种荧光染料染色,并通过扫描激光共聚焦显微镜成像。几种细胞类型特异性或非特异性荧光染料中的一种可以单独使用或组合使用来标记活脑组织中的细胞。荧光缀合的植物isolectin GSA-IB4可用于鉴定小胶质细胞,并跟踪其结构,运动和增殖。活细胞和死亡神经元和神经胶质细胞可以使用膜渗透和不渗透荧光核酸染料区分。非特异性荧光脂质(例如DiIC18)可用作标记内吞和吞噬细胞群体的重要染色剂。使用多通道共聚焦成像,可以在两个或三个空间维度上以及实时地在活体状态下对单标签,双标签或三标签的组织切片进行成像。这提供了研究在各种生理条件下培养的活脑组织中小胶质细胞和其他细胞类型的细胞-细胞相互作用和动态行为的手段。版权所有1999 Academic Press。

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